AU594080B2 - Production of a vitamin c precursor using genetically modified organisms - Google Patents
Production of a vitamin c precursor using genetically modified organisms Download PDFInfo
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- AU594080B2 AU594080B2 AU62210/86A AU6221086A AU594080B2 AU 594080 B2 AU594080 B2 AU 594080B2 AU 62210/86 A AU62210/86 A AU 62210/86A AU 6221086 A AU6221086 A AU 6221086A AU 594080 B2 AU594080 B2 AU 594080B2
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- Prior art keywords
- klg
- dkg
- glucose
- dna sequence
- reductase
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- 125000001449 isopropyl group Chemical group [H]C([H])([H])C([H])(*)C([H])([H])[H] 0.000 description 1
- 229960000274 lysozyme Drugs 0.000 description 1
- 235000010335 lysozyme Nutrition 0.000 description 1
- 239000004325 lysozyme Substances 0.000 description 1
- 229910052943 magnesium sulfate Inorganic materials 0.000 description 1
- 235000019341 magnesium sulphate Nutrition 0.000 description 1
- 235000010355 mannitol Nutrition 0.000 description 1
- 239000000463 material Substances 0.000 description 1
- 238000002844 melting Methods 0.000 description 1
- 230000008018 melting Effects 0.000 description 1
- MYWUZJCMWCOHBA-VIFPVBQESA-N methamphetamine Chemical compound CN[C@@H](C)CC1=CC=CC=C1 MYWUZJCMWCOHBA-VIFPVBQESA-N 0.000 description 1
- 229930182817 methionine Natural products 0.000 description 1
- JZMJDSHXVKJFKW-UHFFFAOYSA-M methyl sulfate(1-) Chemical compound COS([O-])(=O)=O JZMJDSHXVKJFKW-UHFFFAOYSA-M 0.000 description 1
- 230000004048 modification Effects 0.000 description 1
- 238000012986 modification Methods 0.000 description 1
- 238000004713 multireference configuration interaction Methods 0.000 description 1
- VMGAPWLDMVPYIA-HIDZBRGKSA-N n'-amino-n-iminomethanimidamide Chemical compound N\N=C\N=N VMGAPWLDMVPYIA-HIDZBRGKSA-N 0.000 description 1
- 239000002777 nucleoside Substances 0.000 description 1
- 150000003833 nucleoside derivatives Chemical class 0.000 description 1
- 230000003647 oxidation Effects 0.000 description 1
- 238000007254 oxidation reaction Methods 0.000 description 1
- 229910052760 oxygen Inorganic materials 0.000 description 1
- 239000001301 oxygen Substances 0.000 description 1
- NBIIXXVUZAFLBC-UHFFFAOYSA-K phosphate Chemical compound [O-]P([O-])([O-])=O NBIIXXVUZAFLBC-UHFFFAOYSA-K 0.000 description 1
- 239000010452 phosphate Substances 0.000 description 1
- 239000002244 precipitate Substances 0.000 description 1
- 238000007639 printing Methods 0.000 description 1
- 238000011027 product recovery Methods 0.000 description 1
- 230000017854 proteolysis Effects 0.000 description 1
- 150000003212 purines Chemical class 0.000 description 1
- 150000003230 pyrimidines Chemical class 0.000 description 1
- 230000006798 recombination Effects 0.000 description 1
- 238000005215 recombination Methods 0.000 description 1
- BOLDJAUMGUJJKM-LSDHHAIUSA-N renifolin D Natural products CC(=C)[C@@H]1Cc2c(O)c(O)ccc2[C@H]1CC(=O)c3ccc(O)cc3O BOLDJAUMGUJJKM-LSDHHAIUSA-N 0.000 description 1
- 238000011160 research Methods 0.000 description 1
- 238000007480 sanger sequencing Methods 0.000 description 1
- 238000012216 screening Methods 0.000 description 1
- 230000035945 sensitivity Effects 0.000 description 1
- 210000002966 serum Anatomy 0.000 description 1
- 239000001632 sodium acetate Substances 0.000 description 1
- 235000017281 sodium acetate Nutrition 0.000 description 1
- 159000000000 sodium salts Chemical class 0.000 description 1
- 239000000758 substrate Substances 0.000 description 1
- 239000005720 sucrose Substances 0.000 description 1
- 238000003786 synthesis reaction Methods 0.000 description 1
- 238000012360 testing method Methods 0.000 description 1
- 125000003831 tetrazolyl group Chemical group 0.000 description 1
- 229940113082 thymine Drugs 0.000 description 1
- 231100000419 toxicity Toxicity 0.000 description 1
- 230000001988 toxicity Effects 0.000 description 1
- 238000013518 transcription Methods 0.000 description 1
- 230000035897 transcription Effects 0.000 description 1
- 238000000108 ultra-filtration Methods 0.000 description 1
- 241001515965 unidentified phage Species 0.000 description 1
- 238000011144 upstream manufacturing Methods 0.000 description 1
- 229940035893 uracil Drugs 0.000 description 1
- 229940088594 vitamin Drugs 0.000 description 1
- 229930003231 vitamin Natural products 0.000 description 1
- 235000013343 vitamin Nutrition 0.000 description 1
- 239000011782 vitamin Substances 0.000 description 1
- 235000019156 vitamin B Nutrition 0.000 description 1
- 239000011720 vitamin B Substances 0.000 description 1
- 150000003722 vitamin derivatives Chemical class 0.000 description 1
Classifications
-
- C—CHEMISTRY; METALLURGY
- C12—BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
- C12Y—ENZYMES
- C12Y101/00—Oxidoreductases acting on the CH-OH group of donors (1.1)
- C12Y101/01—Oxidoreductases acting on the CH-OH group of donors (1.1) with NAD+ or NADP+ as acceptor (1.1.1)
- C12Y101/01274—2,5-Didehydrogluconate reductase (1.1.1.274), i.e. 2,5-diketo-D-gluconic acid reductase
-
- C—CHEMISTRY; METALLURGY
- C12—BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
- C12N—MICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
- C12N9/00—Enzymes; Proenzymes; Compositions thereof; Processes for preparing, activating, inhibiting, separating or purifying enzymes
- C12N9/0004—Oxidoreductases (1.)
- C12N9/0006—Oxidoreductases (1.) acting on CH-OH groups as donors (1.1)
-
- C—CHEMISTRY; METALLURGY
- C12—BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
- C12P—FERMENTATION OR ENZYME-USING PROCESSES TO SYNTHESISE A DESIRED CHEMICAL COMPOUND OR COMPOSITION OR TO SEPARATE OPTICAL ISOMERS FROM A RACEMIC MIXTURE
- C12P7/00—Preparation of oxygen-containing organic compounds
- C12P7/40—Preparation of oxygen-containing organic compounds containing a carboxyl group including Peroxycarboxylic acids
- C12P7/58—Aldonic, ketoaldonic or saccharic acids
- C12P7/60—2-Ketogulonic acid
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- Chemical Kinetics & Catalysis (AREA)
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- Preparation Of Compounds By Using Micro-Organisms (AREA)
- Enzymes And Modification Thereof (AREA)
- Micro-Organisms Or Cultivation Processes Thereof (AREA)
- Vessels, Lead-In Wires, Accessory Apparatuses For Cathode-Ray Tubes (AREA)
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Abstract
An enzyme for conversion of 2,5-diketo-D-gluconate (2,5-DKG) to 2-keto-L-gulonic acid (2-KLG) and a genetically modified organism that expresses all the fermentation enzymes needed to convert glucose to 2-KLG (a precursor to ascorbic acid) using the new enzyme. Preferably, the organism is Erwinia citreus, or a mutated strain of Erwinia citreus, unable to use 2,5-DKG or 2-KLG as a sole carbon source, into which the gene for a 2,5-DKG reductase, produced by Corynebacterium sp., SHS 752001, has been inserted. The preferred transformed organism expresses the fermentation enzymes Erwinia citreus normally expresses for fermentation of glucose to 2,5-DKG and, in addition, an enzyme Corynebacterium sp. SHS 752001 expresses for fermentation of 2,5-DKG to 2-KLG.
Description
Pci WORLD INTELLECT PR ERTY RGAATIO INTERNATIONAL APPLICATION PUBLISHE N TH PANTO ATION TREATY (PCT) pe i (51) International Patent Classification4 (11) International Publication Number: WO 87/ 00863 C12N 15/00, C12P 19/02 Al (43) International Publication Date: 12 February 1987 (12.02.87) (21) International Application Number: PCT/US84/01571 (72) Inventors; and Inventors/Applicants (for US only) HARDY, Kimber (22) International Filing Date: 1 August 1986 (01.08.86) [GB/CH]; 3, rue Voltaire, CH-1201 Geneva (CH).
VAN DE POL, Hendrick [NL/FR]; 6, all6e du Bois (31) Priority Application Numbers: 8519536 de Graville, F-91190 Gif sur Yvette GRIN- 792,432 DLEY, June [GB/US]; 138 Oak Park Drive, Alameda, CA 94501 PAYTON, Mark, A. [GB/CH]; (32) Priority Dates: 2 August 1985 (02.08.85) 22b, avenue Tronchet, CH-1226 Geneva (CH).
29 October 1985 (29.10.85) (74) Agents: HALEY, James, Jr. et al.; Fish Neave, (33) Priority Countries: GB 875 Third Avenue, New York, NY 10022 (US).
US
(81) Designated States: AT (European patent), AU, BE (Eu- Parent Application or Grant ropean patent), CH,(European patent), DE (Euro- (63) Related by Continuation pean patent), DK, FR (European patent), GB (Euro- US 792,432 (CIP) pean patent), IT (European patent), JP, LU (Euro- Filed on 29 October 1985 (29.10.85) pean patent), NL (European patent), SE (European patent), US.
(71) Applicant (for all designated States except US): 91OG- Published With international search report.
SA b C6'rG k This docufment conta ins thd S14 c-rneM eDG-e cc re amdrnedments riade under cm i t C -rrs oz. Section 49 and is correct for printing.
(54) Title: PRODUCTION OF A VITAMIN C PRECURSOR USING GENETICALLY MODIFIED ORGANISMS (57) Abstract An enzyme for conversion of 2,5-diketo-D-gluconate (2,5-DKG) to 2-keto-L-gulonic acid (2-KLG) and a genetically modified organism that expresses all the fermentation enzymes needed, io convert gluccse to 2-KLG (a precursor to ascorbic acid) using the new enzyme. Preferably, the organism is Erwinia cit, rutited train of Erwinia citreus, unable to use 2,5-DKG or 2-KLG as a sole carbon source, into which the gene for a. redvctase, produced by Corynebacterium sp., SHS 752001, has been inserted. The preferred transformed organis' the fermentation enzymes Erwinia citreus normally expresses for fermentation of glucose to 2,5-DKG an. in enzyme Corynebacterium sp. SHS 752001 expresses for fermentation of 2,5.DKG to 2-KLG.
A.O.J.L 26 i 7
AUSTRALIAN
iMARI 987 PATENT OFRCE _9 i i Cc r r" tf
V-
I"i"'i ;I r4 1 2 WO 87/00863 PCT/S86/01571
-I-
PRODUCTION OF A VITAMIN C PRECURSOR USING GENETICALLY MODIFIED ORGANISMS TECHNICAL FIELD OF THE INVENTION a" This invention relates to DNA sequences, recombinant DNA molecules, organisms containing such sequences and molecules, the expression of certain enzymes by such organisms, and the production, by fermentation, of a Vitamin C precursor using such organisms and enzymes. More specifically, this invention relates to an expression vehicle and genetically modified organisms, transformed by that vehicle, that express enzymes used to convert glucose, or another carbon source, by fermentation to 2-keto-L-gluconic acid (2-KLG), a chemical precursor to Vitamin C (ascorbic acid).
BACKGROUND ART There are several processes for producing Vitamin C. One process involves a number of chemical synthesis steps and one fermentation step. Briefly, the steps are hydrogenation of glucose to sorbitol, fermentation of sorbitol to sorbose using Acetobacter suboxydans, sorbose acetonization, diacetone Morbose oxidation to 2-KLG, esterification of 2-KLG, and conversion of the ester to ascorbic acid. This process is complex and requires a relatively high capital investment for an operating plant.
Vt 'i (i &i ii r. WO 87,"f1863 PCT/S86/01571 -2- Another process involves two fermentation steps. The process starts with fermentation of glucose to 2,5-diketo-D-gluconate (2,5-DKG) by Erwinia sp.; fermentation ofo 2,5-DKG to 2-KLG by Corynebacterium sp.; esterification of 2-KLG; and conversion of the ester to ascorbic acid. ,,One study has shown that D-gluconate and 2-keto-D-gluconate (2-KDG) are produced sequentially from glucose by Erwinia sp. before 2,5-DKG is produced in the first fermentation step. See T. Sonoyama et al., "Production of 2-keto-L-gulonic acid from D-glucose by Two- Stage Fermentation," App. and Envir. Microbiol:, 43, 1064-69 (1982). This two-step fermentation process, although having a somewhat lower capital cost than the Acetobacter process, is still complex and expensive to operate.
Still another process for converting glucose to 2-KLG is referred to in European patent application 132,308. That application refers to the conversion of glucose to 2-KLG in a single step fermentation process. It first refers to Corynebacterium sp. ATCC 31090 as a source of a DNA sequence coding for a particular 2,5-DKG reductase (an enzyme that is said to catalyze the fermentation of 2,5-DKG to 2-KLG). This DNA sequence, with its own or a synthetic ribosome binding site, is then said to be inserted "downstream" of an E.coli trp or tac promoter or the pACYC184 CAT promoter in an expression vector. The vector is also said to contain a gene coding for tetracycline resistance or other selectable marker, and an origin of replication derived from plasmids ColEl, 15A, or RSF 1010. A host cell, Erwinia herbicola (ATCC 21998), is then said to be transformed with the vector. On fermentation this transformed cell is said to produce 2-KLG from glucose in one step. The conversion of glucose to 2-KLG in that process, however, is not fully ~I .2 V;~i 'k
I
kg'' WO 87/00863 PCT/US86/01571 -3satisfactory because the yield of 2-KLG is very-low and the time of fermentation to obtain even that low yield is too long.
Accordingly, a single organism capable of converting a carbon source, such as glucose, to 2-KLG at acceptable rates and in a single fermentation step is still a goal that has not been attained.
SUMMARY OF THE INVENTION The present invention solves the problem of finding a single organism capable of converting glucose, or other carbon source, into 2-KLG quickly and in high yield. In one embodiment, this invention provides an expression vehicle capable of transforming a host so that it performs all of the fermentation steps required for converting glucose, or other carbon source, to 2-KLG in a single fermentation at acceptable conversion rates, without intermediate product recovery or intermediate purification steps. The 2-KLG resulting from practice of the present invention may then be esterified and converted to ascorbic acid (Vitamin as in the conventional processes described above.
In contrast to the process of the present invention, the known commercial fermentation processes for converting glucose to 2-KLG require two separate organisms, for example strains of Erwinia and Corynebacterium, to transform glucose to 2-KLG.
One advantage of the present invention is that a single strain of a genetically modified organism achieves significant yields of 2-KLG directly from glucose in a single fermentation.
Thus, the ability of the process of this invention to use a single fermentation step results in a relatively simpler process than the known commercial
-V
M WO 87/00863 PCT/US86/01571 -17foreign DNA of each of the two recombinant plasmids was 3.0 kb long.
:i WO 87/00863 PCT/US86/01571 -4process so that less process equipment and lessenergy is required to produce Vitamin C from glucose.
Another object of the present invention is to provide a novel'2,5 DKG reductase and a noveltransformed organism superior to those referred to e in European patent application 132,308, and the Sprocesses and products of the present invention are accordingly unexpectedly improved and patentable over the processes and products of European patent application 132,308.
Still other objects and aspects of the invention will be apparent from the specification.
BRIEF DESCRIPTION OF THE DRAWINGS Figure 1 depicts a partial amino acid sequence from the N-terminus of the 2,5-DKG reductase of this invention; Figure 2 depicts part of the amino acid sequence of a 14,000d molecular weight cyanogen bromide fragment of the 2,5-DKG reductase of this invention; Figures 3a-e depict the sequences of several nucleotide probes used to locate by hybridization portions of the Corynebacterium genome containing the 2,5-DKG reductase gene of this invention; and Figure 4 depicts the DNA sequence of the reductase gene of this invention and the corresponding amino acid sequence of the reductase of this invention.
Figure 5 depicts the construction of plasmid pPLred332 from plasmids 210* and pcBR13.
In Figure 5, the symbols have the following meanings: PL, P, promoter; S-D, Shine-Dalgarno sequence; ori, origin of replication; Lac, lac promoter; amp-r, ampicillin resistance gene.
0.
WO 87/00863 PCT/US86/01571 BEST MODE OF CARRYING OUT THE INVENTION In order that the present invention may be more fully understood, the following detailed description is provided. In this specification some of the following terms are employed: Nucleotide A monomeric unit ofoDNA or RNA consisting of a sugar moiety (pentose),oa phosphate, and a nitrogenous heterocyclic base. oThe base is linked to the sugar moiety via the glycosidio carbon carbon of the pentose) and that combination of base and sugar is called 'a nucleoside. The base characterizes the nucleotide. The four DNA bases are adenine guanine cytosine and thymine The four RNA bases are A, G, C, and uracil For DNA, indicates either of the purines (A or indicates either of the pyrimidines (C or and indicates any of the four bases G, C, or For RNA, "IQ,11 and have the same meanings except that "U" is substituted for DNA Sequence A linear array of deoxy nucleotides connected one to the other by phosphodiester bonds between the 3' and 5' carbons of adjacent pentoses.
Codon A DNA sequence of three nucleotides (a triplet) that encodes, through its mRNA, an amino acid, a translation start signal, or a translation termination signal. For example, the nucleotide triplets TTA, TTG, CTT, CTC, CTA, and CTG encode for the amino acid leucine ("Leu" TAG, TAA, and TGA are translation stop signals; and ATG is a translation start signal that also codes for methionine.
Reading Frame The gr.aping of codons during the translation of mRNA into amino acid sequences. During translation the proper reading frame must be maintained. For example, the DNA dan rv sy.'n 1 1 WO 87/00863 PCT/US86/01571 -6sequence GCTGGTTGTAAG may be expressed in three.
reading frames or phases, each of which produces a different amino acid sequence: GCT GGT TGT AAG Ala-Gly-Cys-Lys G CTG GTT GTA AG Leu-Val-Val GC TGG TTG TAA G -Trp-Leu-(STOP) Polypeptide A linear array of amino acids connected one to another by peptide bonds between the a-amino and carboxy groups of adjacent amino acids. When "polypeptide" is used in this specification, it will be understood by those skilled in the art to include the term "protein." Genome The entire DNA of a cell or a virus. It includes, inter alia, the DNA coding for the polypeptides of the cell and operator, promoter, and ribosome binding and interaction sequences, including sequences such as the Shine-Dalgarno sequences for each of those coding sequences.
Gene A DNA sequence that encodes through its template or messenger RNA ("mRNA") a sequence of amino acids characteristic of a specific polypeptide.
Expression The process undergone by a gene to produce a polypeptide. It includes transcription of the DNA sequence to a mRNA sequence and translation of the mRNA sequence -into a polypeptide.
Plasmid A non-chromosomal double-stranded DNA sequence comprising an intact "replicon" such that the plasmid is replicated in a host cell. When the plasmid is placed within a unicellular organism, 30 the characteristics of that organism may be changed or transformed as a result of the DNA of the plasmid.
For example, a plasmid carrying a gene for tetracycline resistance (Tet
R
transforms a cell previously sensitive to tetracycline into one which is resistant to it. A cell transformed by a plasmid is called a "transformant." -1
'*J
-;J-iF ~i' at i 7 a r- -p.i 0 U avs'sw~7-,.,ti WO 87/00863 PCT/US86/01571 -7- Phage or Bacteriophage A bacterial virus.
Many phages consist of DNA sequences encapsulated in protein envelopes or coats ("capsids").
Cloning Vehicle A plasmid, phage DNA, or other DNA sequence that is able to replicate in a host cell. A cloning vehicle is characterized by one or a small number of endonuclease recognition sites at which such DNA sequences may be cut in a determinable' fashion without attendant loss of an essential biological function of the DNA, e.g., replication, production'of coat proteins, or loss of promoter or binding sites. ,A cloning vehicle usually contains a marker suitable for use in the identification of transformed cells, tetracycline resistance or ampicillin resistance. A cloning vehicle is often called a vector.
Cloning The process of obtaining a population of organisms or DNA sequences derived from one such organism or sequence by asexual reproduction.
Recombinant DNA Molecule or Hybrid DNA A molecule, comprising segments of DNA from different genomes joined end-to-end outside of living cells, that may be maintained in living cells.
Expression Control Sequence A sequence of nucleotides that controls and-regulates expression of genes when operatively linked to those genes.
They include the lac system, the p-lactamase system, the trp system, the tac system, the trc systems, the major operator and promoter regions of phage X, the control region of fd coat protein, the early and late promoters of SV40, promoters derived from polyoma virus and adenovirus, metallothionine promoters, the promoter for 3-phosphoglycerate kinase or other glycolytic enzymes, the promoters of acid phosphatase, Pho5, the promoters of the yeast a-mating factors, and other sequences known to control the expression of genes of prokaryotic or c I 1,1 F I WO 87/00863 PCT/US86/01571 -8eukaryotic cells and their viruses or combinations thereof. For mammalian cells the gene can be linked to an eukaryotic promoter such as that for the early region coupled to the gene encoding dihydrofolate reductase and selectively amplified in Chinese hamster ovary cells to produce a cell line containing many copies of actively transcribed eukaryotic genes.
In one embodiment this invention is directed to recombinant DNA molecules, taken-from Corynebacterium s. SHS 752001, characterized by a DNA sequence that codes for the 2,5-DKG reductase of this invention. In another embodiment, this invention is directed to a host, preferably Erwinia citreus, transformed by such a recombinant DNA molecule.
The recombinant DNA molecules of this invention are characterized by a DNA sequence coding for the 2,5-DKG reductase of this invention and an expression control sequence that is operatively linked to that DNA sequence in the recombinant DNA molecule. A wide variety of expression control sequences may be used in the recombinant DNA molecules of this invention. These include the lac system, the P-lactamase system, the trp system, the tac system, the trc systems, the major operator and promoter regions of phage X, the control region of fd coat protein, the early and late promoters of promoters derived from polyoma virus and adenovirus, metallothionine promoters, the promoter I for 3-phosphoglycerate kinase and other glycolytic 30 enzymes, the promoters of acid phosphatase, e.g., the promoters of the yeast a-mating factors, neomycin phosphotransferase promoter, and other sequences known to control the expression of genes of prokaryotic or eukaryotic cells and their viruses or combinations thereof. For mammalian cells, the gene can be linked to an eukaryotic promoter such as that for the SV40 early region coupled to the gene .U WO 87/00863 PCT/US86/01571 -9encoding dihydrofolate reductase and selectively amplified in Chinese hamster ovary cells to produce a cell line containing many copies of it. The preferred expression control sequence of this invention is derived from the lac sequence of pUC8.
In addition, the recombinant DNA molecules of this invention may comprise DNA sequences from a variety of plasmids and phages that allow them to replicate in the chosen host. Preferably, they also include a selection marker, a DNA sequence coding for a drug resistance. Such plasmid and phage sequences may be derived from, for example, segments of chromosomal, non-chromosomal, and synthetic DNA sequences, such as various known derivatives of and known bacterial plasmids, plasmids from E.coli including col El, pCR1, pBR322, pMB9 and their derivatives, wider host range plasmids, RP4, phage DNAs, the numerous derivative of phage A, NM989, and other DNA phages, M13 and Filamenteous single-stranded DNA phages and vectors derived from combinations of plasmids and phage DNAs, such as plasmids which have been modified to employ phage DNA or other expression control sequences or yeast plasmids such as the 2 p plasmid or derivatives thereof.
It should of course be understood that not all vectors and expression control sequences will function in the same way to express the modified DNA sequences of this invention and to produce the new 2,5-DKG reductase of the present invention. Neither will all hosts function equally well with the same expression system. One skilled in the art, however, may make a selection among these vectors, expression control sequences, and hosts without undue experimentation and without departing from the scope of this Sinvention. For example, in selecting a vector, the host must be considered because the vector must S 1 I i l r '-tsr ~i--ULI-.rY_-l PCT/1JS86/01571 WO 87/00863 replicate in it. The vector's copy number, the ability to control that copy number, and°the expression of any other proteins encoded by the vector, such as antibiotic markers, should also be considered.
In selecting an expression control sequence, a variety of factors should also be considered. These include, for example, the relative strength of the system, its controllability, and its compatibility with the DNA sequence encoding the 2,5-DKG reductase of the present invention, particularly as regards potential secondary structures.
The DNA sequence for the 2,5-DKG reductase of this invention may be used to produce that reductase in a wide variety of hosts, bacteria such as strains of E.coli, such as E.coli C600, E.coli ED8767, E.coli DH1, E.coli LE392, E.coli HB101, E.coli X1776, E.coli X2282, E.coli MRCI, and strains of Pseudomonas, Bacillus and Streptomyces, yeasts and other fungi, animal hosts, such as Chinese hamster ovary cells or mouse cells, other animal (including human) hosts, plant cells in culture or other hosts. After expression, the enzyme is then useful for transforming 2,5-DKG to 2-KLG.
Hosts for the DNA sequence of the reductase of this invention generally should be selected by consideration of their compatibility with the chosen vector, the toxicity of the reductase of the present invention to the host, susceptibility of the desired protein to proteolytic degradation by host cell enzymes, contamination or binding of the 2,5-DKG reductase by host cell proteins difficult to remove during purification, expression characteristics, the ability of the host to produce and secrete the 2,5-DKG reductase, the ability of the host to fold the reductase correctly, the fermentation requirements of the host, the ease of
I
i i(:I t t 1~ I I:t r i i WO 87/00863 PCT/US86/01571 -11purification of the 2,5-DKG reductase from the host, safety, and cost.
In one embodiment, Erwinia citreus SHS 2003 is selected as a host because it produces from glucose, and 2-KLG may be produced directly from glucose by a transformedoErwinia citreus SHS 2003.
Most"preferably'hosts of the present invention are Erwinia citreus, SHS2003 (Ferm-P No. 5449; ATCC No. 31623) and a strain mutatedxfrom Erwinia citreus SHS2003, Erwinia citreusI ER1026, that is unable to use either 2,5-DKG or 2-KLG as a sole carbon source.
The following example shows' some embodiments of the invention but is not intended to limit the scope of the'invention.
EXAMPLE
Identification Of A Polypeptide Sequence of the 2,5-DKG Reductase Of This Invention, and Preparation of Cloning Vectors Corynebacterium ap. SHS752001 was described in T. Sonoyama et al., "Production of 2-keto-L-gulonic acid from D-glucose by two-stage fermentation," App. and Envir. Microbiol., 43, 1064-69 (1982).
Thus, the disclosed strain of Corynebacterium, selected as the donor of a DNA sequence coding for a reductase. To aid in identifying the reductase gene from that strain of Corynebacterium, a sample of an enzyme was isolated and purified to 95% purity using the following procedure:o A. Cultivation of Corynebacterium SHS 752001 1. A freeze-dried culture of Co ebacterium sp SHS 752001 was rehydrated immediately after opening by adding 0.4 ml of 0.9% NaCl (sterilized
I
Sia i r, .1 WO 87/00863 PCT/US86/01571 -12at 120 C for 20 minutes) to the contents of a vial containing the freeze-dried culture; 2. The culture was transferred to a test tube containing 8 mls of a solution containing glucose, 0.5% yeast extract (Difco), 0.5% peptone (Difco), 0.1% KH2PO4, 0.02% MgSO4*7H20 and 2.0% agar.
The solution pH was 7.0, and the solution had been sterilized at 120 0 C for 15 min. Forty hours after the addition of the culture at 28 0 C, the culture was suspended with 0.4 ml of 0.9% NaCl that had been sterilized at 120°C for 20 min.; 3. Five lots of 0.1 ml of the suspension from step 2 were added to five agar slants containing the same ingredients as the solution of step 2. The cultures were fermented for the same amount of time and under the same conditions as step 2. The cultures were suspended with 5 ml of 0.9% NaCl (sterilized at 120 0 C for 20 min.), and 2.5 ml of the suspension was transferred to a each of ten seed flasks containing 500 ml of medium.
4. A solution containing: 1% glucose, yeast extract (Difco), 0.5% peptone (Difco), 0.1% NaNO 3 0.1% KH 2
PO
4 and 0.02% MgSo 4 *7H 2 0, and having a pH of 7.0 was sterilized at 120 C for 15 minutes. Sixty ml of the solution were added to a 500ml flask containing the culture. After 16-18 hours of cultivation at 28 0 C, the culture content of 10 such 500 ml flasks were transferred to a 30 liter jar fermentor; and 5. Twenty liters of a solution at pH 7.2, containing 1.8% glucose, 2.7% corn steep liquor 0.31% NaNO 3 0.06% KH 2
PO
4 4.4 ppm ZnSO 4 7H 2 0, 0.72 ppm MnCI2-4H 2 0, 0.2 ppm Vitamin B -HC1, 0.15 ppm Calcium panthothenate, and 0.005% antiform (Adekanol), was added to the 30 liter jar fermentor containing the culture. The fermentor was incubated at 28 0 C with agitation at 400 rpm and an air flow rate of -wT
I
Ki -cv~ a Cr i:il WO 87/00863 PCT/US86/01571 -13- The fermentation was stopped when glucose disappeared from the culture (22h). The final pH was 7.5 and the final OD was 19.2.
B. Preparation of cell extract About 750 gr of cells were harvested from the 30 liter jar fermentor by centrifugation using a.
Sharples centrifuge (10,000 G, 10 minutes). The cells were suspended in 0.1M tris-HCl buffer (pH 7, washed three times with the same buffer (2.5 L in each case) using a centrifuge, and finally resuspended in 1.6 L of the buffer (OD 150). The cells (as 80 ml of cell suspension) were disrupted by sonication (160 watts for 7 min.). Unbroken cells and debris were removed by centrifugation (15,000 G for 30 min.), and the supernatant (1 L) was pooled.
C. Fractionation by AmSo 4 The protein material that precipitated between 40% and 70% saturation was collected by centrifugation, and redissolved in 80 mls of 0.1 M tris-HCl buffer at pH 7. The solution was dialyzed against 0.02 M tris-HCl buffer at pH 7 overnight.
D. Ion-Exchange Chromatography The dialyzed solution (99 ml) was placed on a DEAE-Sepharose CL-6B column (1.6 x 30 cm) previously equilibrated with 0.02 M tris-HCl buffer (pH7). The column was washed stepwise with 0.02 M tris-HCl buffer containing zero and 0.2 M NaCl (pH The enzyme was eluted with the same buffer containing 0.3 M NaC1 (pH The active fractions were pooled and the protein was conc~ntrated by adding AmSO 4 up to 70% saturation. The precipitate was collected and dialyzed as in step C.
L.
1 1 i r a~ 7 -::;r;;:,I~~aiaw~iLus;rmu*w~ WO W,7/oo863 PCT/US86/01571 -14- E. First Affinity Chromatography The dialyzed solution (37 ml) obtained from step D was placed on an Amicon Matrix Red A column (1.6 x 19 cm) previously equilibrated with 0.02 M tris-HCl buffer (pH The column was washed stepwise with 0.02M tris-HCl buffer (pH 7) containing 0.3 -0.5M NaCl. The enzyme was eluted with the same buffer containing 0.7-1.OM NaCl.
The active fractions (90ml) were pooled.
F. Second Affinity Chromatography 0.02M tris-HCl buffer (pH 7, 225 ml) was added to the pooled fraction from step E, and the resulting solution was placed on an Amicon Matrix Red A column (1.9 x 12.3 cm) previously equilibrated with 0.02 M tris-HCl buffer (pH The column was washed with 0.02 M tris-HCl buffer (pH 7) containing 0.2M NaCl. The enzyme was eluted with the same buffer containing 0.5 mM NADPH. The active fractions (35 ml) were pooled and concentrated by ultra-filtration (cut-off below M.W. of 10,000) to remove NADPH.
To demonstrate that the 2,5- DKG reductase of this invention was hot denatured during the sonication process and to confirm that the 2,5-DKG reductase of this invention converts 2,5-DKG to 2-KLG, a mixture of 0.1M tris-HC1 (pH7) was prepared containing 7 mg NADPH, 2 mg 2,5-DKG and 50 pl cell sonicate at a total protein concentration of 2.5 mg/pl. The total reaction volume was 200 pl. The products of the reaction were analyzed by HPLC, and the presence of 30 2-KLG was confirmed.
Antibodies to the 2,5-DKG reductase of this invention were prepared. The antibodies were developed by injecting a rabbit intradermally at multiple sites with 100 pg of the 2,5-DKG reductase of this invention in Freunds adjuvant and boosting ,1 :i i i-i .f .:i iv r WO 87/00863 PCT/US86/01571 with 50 pg of the enzyme in Freunds incomplete solution twenty-one days later. Serum was taken ten days after the boost injection and was shown to be positive for anti-(2,5-DKG reductase of this invention) activity in an enzyme-linked immunoabsorbant ("ELISA") assay.
The purified enzyme was sequenced from the N-terminus using a high sensitivity gas phase sequenator manufactured by Applied Biosystems. The partial sequence obtained by this method is shown in Figure 1. A question mark in the Figure indicates that a particular amino acid could not be determined with absolute certainty.
The purified enzyme was also cleaved using a standard cyanogen bromide clevage procedure. A portion of the amino acid sequence of one 14,000d fragment produced by that method is shown in Figure 2.
In order to select from a library of clones a DNA sequence coding for that 2,5-DKG reductase of this invention, a series of oligonucleotlde probes (shown in Figures 3a-e) was prepared, using the phosphotriester method. These probes were derived from the amino acid sequences of Figures 1 and 2.
Because of the degeneracy of the genetic code, each probe was actually a family-of structurally related molecules. For example, the 14-mer DNA probe of Figure 3a (Probe I of Figure 1) had a redundancy of 96 with one C-T mis-match over the predicted sequence, the 14-mer DNA probe of Figure 3b (Probe II of Figure 1) had a redundancy of 32 with Sone G-T mis-match, the 17-mer DNA probes of Figures 3c and 3d (Probe III of Figure 1) each had a redundancy of 32 and differed from one another only in the first two positions, and the 14-mer DNA probe of Figure 3e (Probe IV of Figure 2) had a redundancy j of 32.
WO 87/00863 PCT/US86/01571 -16- To construct libraries of Corynebacterium DNA to permit screening by the probes of Figures 3(a-e) to select the 2,5-DKG reductase gene of this invention, Corynebacterium sp. SHS 752001 was lysed by treating a cell suspension of Corynebacterium sp. SHS 752001 with lysozyme (1 mg/1) in 10 mM Tris-HCl (pH 1 mM EDTA and 20% (w/v) sucrose followed by sodium dodecylsulfate (SDS) mg/ml). DNA from the lysed Corynebacterium sp.
SHS 752001 cells was then fragmented using the restriction endonuclease Sau3a in a buffer comprising 150 mM NaCI, 6 mM Tris-HCl (pH 6mM MgCl 2 and 100 pg/ml bovine serum albumin. The DNA fragments were then inserted into pUC8 vectors at a BamHl site using the method of J. Viera and J. R. Messing, Gene, 19, 259 (1982), and the recombinant plasmids were transformed into Escherichia coli JM83, W 3 110 i q and W 3 1 1 0 i recA. The method for transformation of the recombinant plasmids into E.coli JM83 is set forth in J. R. Messing, R. Corea, P. H. Seeburg, Nucleic Acids Res., 9, 309 (1981). Similar methods were used for other host strains.
Colonies of the resulting library were screened with the probes of Figures 3(a-e) using the procedure set forth in Wallace, B.,-Johnson, M. Hirose, Miyake, Kawashima, E. H. and Itakura, Nucleic Acids Res., 9, 879-94 (1981).
The probes were hybridized at 37°C and were also Swashed at 37 0 C in a standard wash comprising 6 x SSC, 5 x Denhardt's buffer, 0.1% SDS, and pg/ml t-RNA. Of seventeen colonies that were positive (hybridized) with the probe of Figure 3e, two were also positive with the probes of Figures 3c or 3d or both. The two recombinant plasmids of those clones were designated pCBR0 and pCBR13. The
S.,
L
i i WO 87/00863 PCT/US86/01571 -17foreign DNA of each of the two recombinant plasmids was 3.0 kb long.
Properties of Expression Vectors and Transformants According To the Invention In order to determine the properties of the recombinant plasmids, including production rates of the 2,5-DKG reductase of this invention by the transformed hosts, the two recombinant plasmids and pUC8, a vector not containing the DNA coding for the 2,5-DKG reductase of this invention, were transformed into E.coli W3 11 0i recA and Erwinia punctata by the procedure set forth in Cohen, S. Chang, A. C. Y., and Hsu, Proc. Natl. Acad. Sci. USA, 69, 2110 (1972)). Vector pUC8, which is related to pBR322, has a strong lac promoter located slightly upstream from a BamHl site.
Several procedures were examined for releasing the 2,5-DKG reductase of this invention from the transformed cells that produced it so that production rates could be measured. Sonication was found to be best for E.coli and Erwinia.
Extracts of E.punctata and of E.coli carrying pCBR10 and pCBR13 were analyzed by sodium dodecylsulfate-polyacrylamide gel electrophoresis (SDS-PAGE) (Laemmli, U. K. Nature, 227, 680-85 (1970)) and by Western blotting (Thomas, P. S., Proc. Natl. Acad. Sci. USA, 77, 5201-05 (1980)) using reductase of this invention) antibody, produced above, to determine the amount of reductase of this invention produced by the transformants. Extracts of E.coli W3 110 iq recA (pCBR13) treated with the lac inducer isopropyl P-D-thiogalactopyranoside (IPTG) contained about five times more enzyme than extracts from uninduced cells with N35 the plasmid carrying the gene.
1 1 1 :i r 1 ii i WO 87/00863 PCT/US86/01571 -18- Confirmation that the Reductase of this Invention was not Altered During Recombination The 2,5-DKG reductase produced by E.punctata and E.coli after transformation with pCBRO and pCBR13 was examined to see if it was the same enzyme isolated from Coyrnebacterium sp.
SHS 752001.
The molecular weight of the protein, labelled by Western blotting of extracts of Erwinia (pCBR13), of E.coli W 3110 q recA (pCBR13), and of Corynebacterium, was the same as the molecular weight of the purified 2,5-DKG reductase of this invention about 29,000d). Based on comparison of the blots for the different cells, it was estimated that 1-2% of the total cell protein of Erwinia (pCBR13) was the 2,5-DKG reductase of this invention.
We have made further constructions using the AlL promoter, a strong promoter which can be controlled by the XcI repressor protein. Expression of the APL promoter can be controlled by changing the temperature from 30 0 C to 420C in a strain which also carries the ACI857 temperature-sensitive repressor.
Increased yields of 2-KLG from recombinant strains were obtained using this promoter system.
Figure 5 shows the physical map of the 'vector used for making the plasmids expressing reductase under the control of the APL promoter.
Plasmid pPLred332 was made by inserting the fragment coding for 2,5-DKG reductase from plasmid pCBR13 into plasmid p210*. The fragment inserted was generated by digestion of pCBR13 with restriction endonucleases F EcoRI and HindIII; the two fragments were separated by electrophoresis through low melting agarose. The vector was also digested with EcoRI and HindIII (see Figure 5) so that the appropriate fragments could be ligated. The resulting plasmid, pPLred332, was -a II: -I l Ili 7 WO 87/00863 PCT/US86/01571 -19transformed into strain W3110 cIts to form strain EC1083. This strain carries a chromosomal insertion of the lambda temperature-sensitive repressor gene cl857. Plasmid pPLred332, which comprises the vector element derived from 210* and the insert from pCBR13 Sas shown in Figure 5, specifies 2,5-DKG reductase which has the same molecular weight, in both E.coli and in Erwinia citreus, as that specified by pCBR13.
Erwinia citreus ER1026 was transformed with pPLred332 to form strain E1116.
In order to confirm the amino acid and DNA sequence of the 2,5-DKG reductase of this invention, the 3 kb insert of pCBR13 was sequenced by the Maxam and Gilbert technique (Proc. Natl. Acad. Sci. USA, 74, 560 (1977) and Maxam, A. M. and Gilbert, W., Meth. Enzym., 65, 499-560 (1980)) and by Sanger sequencing using plasmid M13 (Sanger, Nickelen, S.
and Coulsen, A. Proc. Nat'l Acad. Sci. U.S.A., 74, 5463-67 (1977)). Examination of the sequence of the 3.0 kb insert revealed a sequence that code6C almost exactly for the first sixty amino acids determined for the enzyme itself (as shown in Figure 1).
The 3.0 kb insert also contained a sequence that coded almost exactly for the amino acid sequence of Figure 2. The end of the reductase gene in the kb insert was indicated by a STOP codon. In this way the reductase gene was determined to be 831 nucleotides long (omitting the STOP codon and including ATG, the START codon), and its sequence is shown in Figure 4.
The DNA sequence coding for the amino acid sequence of the 2,5-DKG reductase of this invention may be compared to the DNA sequence coding for, and the amino acid sequence of, the polypeptide of European Patent Application 132,308. Figure 4 shows both the DNA sequence and amino acid sequence for the 2,5-DKG reductase of this invention. Figure 4 11 iI.-- ^I i ii- 'P II WO 87/00863 PCT/US86/01571 of European Patent Application 132,308 shows the purported DNA sequence and amino acid sequence of that polypeptide. A comparison of the two figures clearly shows that the 2,5-DKG reductase of this invention and its DNA sequence are markedly different from the amino acid sequence and DNA sequence of European Patent Application 132,308.
The Michaelis constant (Km) of an enzyme measures the kinetics of that enzyme. The lower the value of the constant, the higher the activity, or velocity, of the enzyme. The Michaelis constant for the 2,5 DKG reported in European Application 132,308 is 15.5 mM, and the Michaelis constant for the DKG reductase of this invention (using 100 pM NADPH as a cofactor) in 0.1 M Tris-HCl, pH 7.0 at is 2.0 mM.
The following procedures illustrate fermentation of glucose to 2-KLG, a Vitamin C precursor, using a genetically modified organism of this invention.
Fermentation of Glucose to 2-KLG Using Transformed Erwinia Erwinia citreus SHS 2003, c.i deposit with the-American Type Culture Collection, Maryland, ATCC No. 31623 and on deposit with the Fermentation Research Institute, Yatabe, Japan, FERM-P No. 5449, normally expresses enzymes for converting glucose to 2,5-DKG. This strain was transformed with pCBR13, which, as described above, contains a gene that codes for the 2,5-DKG reductase of this invention, using the procedure set forth in J Cohen, S. Chang, A. C. and Hsu, Proc.
Nat'l. Acad. Sci. USA, 69, 2110 (1972). The resulting strain, designated ER817, thus should contain the genes for all the enzymes required for converting glucose to 2-KLG in a single fermentation.
SI i a l l l 1 1 .:i 1 1 1 r-4 WO 87/00863 PCT/LS86/01571 -21- Strain ER817 was inoculated onto a plate of L-broth agar that contained ampicillin (40 pg/ml).
The strain had been taken from a stock culture kept in L-broth plus 15% glycerol at -70 0 C. After the plate had undergone 24 hours incubation at 18 0
C,
ml of a seed medium (glycerol, 5 g/l; corn steep liquor, 27.5 g/l; KH 2
PO
4 1 g/l; pH 6.8) in a 250 ml conical flask was inoculated to an absorbance at 650 mm of 0.05 (A 650 0.05) with strain ER817 taken from the plate.
The resulting seed culture was incubated for 24 hours at 18°C with rotary shaking. Ten ml of a production medium (corn steep liquor, 30 g/1;
KH
2
PO
4 1 g/l; NaC1, 1 g/1; CaCO 3 29 g/l; glucose, 10 g/l; pH 6.8) in a 250 ml conical flask was inoculated to A650 0.2 with the seed culture and was incubated with rotary shaking at 28 0 C for 65 hours.
The culture was then centrifuged and the supernatant was analyzed for the presence of 2-KLG by high performance liquid chromatography (HPLC).
Fifty pl samples of the supernatant were analyzed using a Biorad HPX-87H column at 65 0 C (0.6 ml/min) in 0.18N H 2
SO
4 A peak having a retention time of 8.86 min indicates the presence of 2-KLG. The retention times of the other compbunds of interest are as follows: 2,5-DKG, 8.46 min; 2-keto-D-gluconic acid (2-KDG), 9.20 min; gluconic acid, 10.0 min; and fucose, 12.1 min.
The various samples of supernatant showed a peak at 8.86 min, indicating the presence of 2-KLG at a concentration of 1 g/1. To confirm that the compound producing a peak at 8.86 min was 2-KLG, a quantity of known 2-KLG (as the sodium salt) was added to a sample of supernatant. That increased only the peak at 8.86 min, thereby providing the confirmation sought. In contrast, when a sample of culture was taken only 18 hours after inoculation q VO 87/00863 PCT/US86/01571 -22- (rather than after 65 hours), HPLC analysis of -the supernatant contained 2,5-DKG in a concentration of 7 g/l, but no detectable 2-KLG.
To confirm further that 2-KLG (and not 2-KDG) was actually being produced in the culture, a quantity of known 2-KDG (as the calcium salt) was added to a sample of the supernatant to a concentration of 1 g/l. HPLC analysis of that spiked culture then showed the presence of a new peak at 9.16 min, but essentially no change in the 2-KLG peak at 8.86 min.
Another method of demonstrating the production of 2-KLG by the culture was also used. By converting any 2-KLG produced by the fermentation to ascorbic acid, a reducing agent, the reducing capacity of a fermentation medium containing 2-KLG may be measured, and the amount of 2-KLG present in the solution before its conversion to ascorbic acid may be calculated. To compensate for the presence of reducing agents other than ascorbic acid in a fermentation mixture, a first sample of a fermentation mixture is treated to convert 2-KLG to ascorbic acid and then the total reducing capacity of the sample is determined. A second sample is prepared that, after conversion of the 2-KLG, has had all ascorbic acid eliminated from the medium. The reducing activities of the two samples are then compared, and the difference in activity should indicate the amount of ascorbic acid present in the samples, and hence the 2-KLG present in the fermentation medium.
A sample of supernatant of a fermentation medium was treated to convert any 2-KLG present into Vitamin C. 75 pl of 8N HC1 were added to 50 pl of the supernatant and the mixture was incubated for min at 95 0 C. 120 pl of 5N NaOH were added and the pH was adjusted to 3.75 using 1 N sodium acetate.
-i i, 1 1 1 1
I
4 1 WO 87/00863 PCT/US86/01571 -23- Ascorbic acid and any other reducing agents in the mixture would reduce the tetrazolium salt MTT [3-(4,5-dimet:hylthiazolyl-2)-2,5-diphenyltetrazolium bromide] in the presence of the electron carrier PMS [5-methylphenazium methylsulphate] to a formazan.
Such treatment was carried out and it indicated the total of all reducing agents (including Vitamin C) in the mixture.
To facilitate specific determination of Vitamin C, a sample of the fermentation mixture before treatment with MTT and PMS was treated with ascorbic acid oxidase and oxygen to destroy any Vitamin C present. Subsequent treatment with MTT and PMS then indicated the amount of reducing agents other than Vitamin C present, and by difference the amount of Vitamin C (and thus of 2-KLG) was determined. In this way the presence of Vitamin C in the mixture and, therefore, the presence of 2-KLG in the supernatant were proven.
Using the procedure for converting 2-KLG to Vitamin C with samples containing known concentrations of 2-KLG allowed preparation of a standard curve. The curve showed that the supernatant obtained from the 65-hour culture of strain ER817 contained 1 g/l of 2-KLG, agreeing with results of the HPLC analyses. 2-KLG was not detected in the supernatant of a similarly produced and treated culture of another strain of Erwinia citreus that lacks pCBR13 (strain SHS2003).
Conversion of glucose to 2-KLG was carried out with the following fermentation procedure using transformed strain ER817. Inoculation was carried out as in Example 1 but incubation in the production medium was for 30 hours instead of for 65 hours and 100 ml of culture were used. The culture supernatant contained 1 g/l of 2-KLG but less than 0.1 g/l of' glucose, 2-KDG, 2,5-DKG, or gluconic acid.
i !w 44 7-w^m WO 87/00863 PCT/US86/01571 -24- One way of obtaining better yields of 2-KLG is to ensure that none of the intermediates produced in the fermentation of glucose to 2-KLG are being consumed in biological reactions that are unrelated to 2-KLG production. Accordingly, a mutant of Erwinia citreus (SHS2003) that was unable to use 2,5-DKG or 2-KLG as sole carbon source was isolated following nitrosoguanidine mutagenesis in the procedure described by Miller, Experiments in Molecular Genetics (Cold Spring Harbor, 1974), except that the cells were incubated in the presence of nitrosoguanidine at After mutagenesis, the cells were incubated for 18h at 30 0 C in M9 medium, that contained glucose (0.2% w/v) or glycerol w/v) as described in Miller, Experiments in Molecular Genetics (Cold Spring Harbor, 1974). Samples of the culture were spread onto plates of M9 glucose or M9 glycerol medium and were then replicated onto plates of M9 medium containing w/v) or 2-KLG Mutants unable to grow on either of these media were purified by restreaking and were tested for their ability to use a variety of substrates as sole carbon sources.
Several mutants were obtained that could not use any of 2,5-DKG, 2-KDG or 2-KLG as sole carbon sources.
One such mutant was transformed with plasmid pCBR13 to form strain ER1037, which was then tested for its ability to convert glucose to 2-KLG.
A culture of Erwinia citreus ER1037 was deposited in the 7 eutsch Sammlung von Mikroorganismen culture collection. The culture was deposited on July 22, 1985 and is identified as follows: DSM No. 3404.
A culture of strain ER 1037 was grown for 18h in L-broth and 90 ml of this culture was inoculated into 500 ml of a medium comprising (per liter): K2HPO4, 4g; KH2PO4, g1; NH4C1, Ig; CaC12, 0.Olg;
K
2
SO
4 2.6g; casamino acids, 10g; yeast extract, -1 11 i i _il WO 87/00863 PCT/US86/01571 corn steep liquor, 10g; D-mannitol, 20g; and glucose, 10g. After 20h growth at pH 6.0 in a 1 liter fermentor (aeration at 0.7 vessel volumes min- agitation at 800 the concentration of 2-KLG in-the growth medium was 6.25 g/liter.
Using"Erwinia citreus ER1026 transformed with the plasmid pPLred332, a further improvement in yield of 2-KLGvcan be achieved. The resulting strain, ER1116, iLs'grown as described above. However, instead of terminating the fermentation described in the example after 20 h, the fermentation was extended by the addition of a further 10 g/L of glucose 12 h after inoculation.
Two further additions of 10 g/L of glucose can also be made 36 h and 60 h after the start of the fermentation. A final level of 2-KLG in the fermentation broth was 19.83 g/L representing a conversion from glucose of 49.4%.
It will be apparent to those skilled in the art that various modifications may be made in the invention without departing from its scope or spirit, and our basic construction can be altered to provide other embodiments which utilize the processes and compositions of this invention. Therefore, it will be appreciated that the scope of this invention is to be defined by the claims appended hereto rather than the specific embodiments which have been presented Sas examples.
Claims (17)
1. A DNA sequence coding for a redqctase as hereinbef ore defined, said DNA sequence selected from the group consisting of: a DNA sequence of the formula: CCGAACATCCCCACCATCAGCCTCAACGACGGACGCCCCTTCGCCGAG CCTGGGCTCGGCACGTACAACCTGCGCGGCGACGAGGG%-GGTCGCGGCCATG GTCGCCGCGATCGACTCGGGCTACCGCCTGCTCGACACGGCGGTGAACTAC GAGAACGAGAGCGAGGTCGGCCGAGCGGTGCGCGCGAGCAGCGTCGATCGC GACGAGCTCATCGTGGCGAGCAAGATCCCGGGCCGCCAGCACGGGCGCGCC GAGGCGGTCGACAGCATCCGCGGATCGCTCGACCGGCTGGGGCTCGACGTG ATCGACCTGCAGCTGATCCACTGGCCGAACCCCAGCGTGGGCCGGTGGCTC GACACCTGGCGCGGCATGATCGACGCGCGCGAGGCGGGCCTGGTCCGCTCG ATCGGCGTCTCGAACTTCACCGAGCCGATGCTGAAGACCCTCATCGACGAG ACCGGGGTCACACCCGCGGTCAACCAGGTCGAGCTCCACCCGTACTTCCCC CAGGCGGCGCTGCGCGCGTTCCACGACGAGCACGGCATCCGCACCGAGAGC **:TGGAGCCCGCTCGCCCGGCGCAGCGAGCTGCTCACCGAGCAGCTGCTCGCAG *see GAGCTGGCGGTCGTCTACGGAGTGACGCCGACGCAGGTGGTGCTGCGGTGG 0:000:CACGTGCAGCTCGGCAGCACCCCGATCCCCAAGTCCGCCGACCCCGATCGC CAGCGCGAGAACGCCGATGTGTTCGGCTTCGCCCTCACCGCCGACCAGGTC 00 @0 ACGCACGAAGAGATG; and DNA sequences w~hich, as a result of egOSthe degeneracy of the genetic code, code for a polypeptide specified by the foregoing DNA sequence.
A recombinant DNA molecule comprising a ~.DNA sequence coding for a 2,5-DKG reductase as hereinbefore defined, said DNA sequence selected from 06 the group consisting of: a DNA sequence of the formula: 0 CCGAACATCCCCACCATCAGCCTCAACGACGGACGCCCCTTCGCCGAG 0 0 0 CCTGGGCTCGGCACGTACAACCTGCGCGGCGACGAGGGGGTCGCGGCCATG GTCGCCGCGATCGACTCGGGCTACCGCCTGCTCGACAC-GCGGTGAACTAC a t -J4 i 27 GAGAACGAGAGCGAGGTCGGCCGAGCGGTGCGCGCGAGCAGCGTCGATCGC GACGAGCTCATCGTGGCGAGCAAGATCCCGGGCCGCCAGCACGGGCGCGCC GAGGCGGTCGACAGCATCCGCGGATCGCTCGACCGGCTGGGGCTCGACGTG ATCGACCTGCAGCTGATCCACTGGCCGAACCCCAGCGTGGGCCGGTGGCTC GACACCTGGCGCGGCATGATCGACGCGCGCGAGGCGGGCCTGGTCCGCTCG ATCGGCGTCTCGAACTTCACCGAGCCGATGCTGAAGACCCTCATCGACGAG ACCGGGGTCACACCCGCGGTCAACCAGGTCGAGCTCCACCCGTACTTCCCC CAGGCGGCGCTGCGCGCGTTCCACGACGAGCACGGCATCCGCACCGAGAGC TGGAGCCCGCTCGCCCGGCGCAGCGAGCTGCTCACCGAGCAGCTGCTGCAG GAGCTGGCGGTCGTCTACGGAGTGACGCCGACGCAGGTGGTGCTGCGGTGG CACGTGCAGCTCGGCAGCACCCCGATCCCCAAGTCCGCCGACCCCGATCGC CAGCGCGAGAACGCCGATGTGTTCGGCTTCGCCCTCACCGCCGACCAGGTC GATGCGATCTCGGGCCTCGAGCGCGGGCGGCTCTGGGACGGCGACCCCGAC ACGCACGAAGAGATG; and DNA sequences which, as a result of the degeneracy of the genetic code, code for a polypeptide specified by the foregoing DNA sequence.
3. The recombinant DNA molecule of claim 2, wherein said DNA sequence is operatively linked to an expression control sequence in the molecule.
4. The recombinant DNA molecule of claim 3, wherein said expression control sequence is selected from the group consisting of the lac system; the B-lactamase system; the trp system; the tac system; the trc system, the major operator and promoter regions of phage A; and the control region of fd coat protein, the early and late promoters of SV4O, promoters derived from polyomavirus and adenovirus, metallothiomine promoters, the promoter for 3-phosphoglycerate kinase or other glycolytic enzymes, the promoters of acid phosphatase, the promoters of the yeast a-mating factors; promoters for mammalian cells such as the early and late promoters, adenovirus late promoter, and 0SS@ 0 0 0000 0 4 -4 00000 6 OS0 0 0 0 0 000 0 0 0 0 s @00 1' 0 0 S 00 0 0 S @500 05 0 I i t j0 1 O 00 0 S 4, mf -28- other sequences that control the expression of genes of prokaryotic or eukaryotic cells and their viruses and combinations thereof.
A transformant. comprising a host trans- formed with at least one recombinant DNA molecule according to claim 3 or 4.
6. The transformant of claim 5, wherein said host makes 2,5-diketo-D-gluconic acid.
7. The transformant of claim 6, wherein said host belongs to the genus Erwinia.
8. The transformant of claim 6, wherein the host is Erwinia citreus.
9. A 2,5-DKG reductase as hereinbefore Seesdefined selected from the group consisting of: a 2,5-DKG reductase having the amino 0 acid sequence: :0 ProAsnl leProThrl leSerLeuAsnAspGlyArgProPheAlaGluPro GlyLeuGlyThrTyrAsnLeuArgGlyAspGluGlyVa lAlaAlaMetVa
1 0 AlaAlaI leAspSerGlyTyrArgLeuLeuAspThrAlaValAsnTyrGlu *AsnGluSerGluValGlyArgAlaValArgAlaSerSerValAspArgAsp GluLeuIleValAlaSerLysIleProGlyArgGlnHisGlyArgAlaGlu AlaValAspSerI leArgGlySerLeuAspArgLeuGlyLeuAspVallle O AspLeuGlnLeul leHisTrpProAsnProSerValGlyArgTrpLeuAsp ThrTrpArgGlyMetlleAspAlaArgGluAlaGlyLeuValArgSerlle GlyValSerAsnPheThrGluProMetLeuLysThrLeul leAspGluThr GlyValThrProAlaValAsnGlnValGluLeuHisProTyrPheProGln AlaAlaLeuArgAlaPheHisAspGluHisGlylleArgThrGluSerTrp SerProLeuAlaArgArgSerGluLeuLeuThrGluGlnLeuLeuGlnGlu LeuAlaValValTyrGlyVa lThrProThrGlnValValLeuArgTrpHis ~Va lGlnLeuGlySerThrProl leProLysSerAlaAspProAspArgGln rviA LL I -29 ArgGluAsnAlaAspValPheGlyPheAlaLeuThrAlaAspGlnValAsp AlalleSerGlyLeuGluArgGlyArgLeuTrpAspGlyAspProAspThr HisGluGluMet; and a 2,5-DKG reductase having the amino acid sequence of and additionally including methionine residue at its amino end. A 2,5-DKG reductase as hereinbefore defined produced by the transformant of claim
11. A method for producing a reductase as hereinbefore defined comprising culturing a host transformed by a recombinant DNA molecule according to claim 2 or 3.
12. The method of claim 11, further comprising the step of isolating said reductase.
13. A process for producing 2-KLG as hereinbefore defined from glucose comprising the step of fermenting the transformant of claim 8 in a medium comprising glucose. S.
14. A process for producing vitamin C, comprising the steps of: fermenting the transformant of Sclaim 6 in a medium comprising glucose to produce 2-KLG; and converting said 2-KLG to vitamin C. I
15. The transformant of claim 8, wherein said host is selected from the group consisting of S Erwinia citreus SHS2003 and Erwinia citreus ER 1026. L ®Xt k I I
16. A process for producing 2-KLG from glucose comprising the steps of: isolating a mutant of Erwinia unable to use 2,5-DKG as the sole carbon source; transforming said mutant with a recombinant DNA molecule comprising a DNA sequence of claim 1 operatively linked to a lambda P, promoter; and fermenting said mutant in a medium comprising glucose.
17. The process of claim 17, wherein the pH of said medium is maintained at about pH DATED this 7th day of September 1989 BIOGEN, N.V. By their Patent Attorneys G.R. CULLEN CO. S S em S 0 00 S S,. 469S6 so 0 0 *000 i S. "I jiis a j. t i:i s; i t- i;
Applications Claiming Priority (4)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| GB858519536A GB8519536D0 (en) | 1985-08-02 | 1985-08-02 | Vitamin c precursor |
| GB8519536 | 1985-08-02 | ||
| US79243285A | 1985-10-29 | 1985-10-29 | |
| US792432 | 1985-10-29 |
Publications (2)
| Publication Number | Publication Date |
|---|---|
| AU6221086A AU6221086A (en) | 1987-03-05 |
| AU594080B2 true AU594080B2 (en) | 1990-03-01 |
Family
ID=26289601
Family Applications (1)
| Application Number | Title | Priority Date | Filing Date |
|---|---|---|---|
| AU62210/86A Ceased AU594080B2 (en) | 1985-08-02 | 1986-08-01 | Production of a vitamin c precursor using genetically modified organisms |
Country Status (7)
| Country | Link |
|---|---|
| EP (1) | EP0231354B1 (en) |
| JP (4) | JPH0817706B2 (en) |
| AT (1) | ATE78297T1 (en) |
| AU (1) | AU594080B2 (en) |
| DE (1) | DE3686041T2 (en) |
| DK (1) | DK175120B1 (en) |
| WO (1) | WO1987000863A1 (en) |
Families Citing this family (10)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| US5008193A (en) * | 1984-06-14 | 1991-04-16 | Genentech, Inc. | Ascorbic acid intermediates and process enzymes |
| US5032514A (en) * | 1988-08-08 | 1991-07-16 | Genentech, Inc. | Metabolic pathway engineering to increase production of ascorbic acid intermediates |
| US5376544A (en) * | 1992-09-08 | 1994-12-27 | Rutgers The State University Of New Jersey | Enzymes for the production of 2-keto-L-gulonic acid |
| US5795761A (en) * | 1996-01-11 | 1998-08-18 | Rutgers, The State University Of New Jersey | Mutants of 2,5-diketo-D-gluconic acid (2,5-DKG) reductase A |
| US6916646B1 (en) * | 1997-06-23 | 2005-07-12 | Genencor International, Inc. | Enterobacteriaceae fermentation strains |
| US6407046B1 (en) | 1998-09-03 | 2002-06-18 | Genencor International, Inc. | Mutant EGIII cellulase, DNA encoding such EGIII compositions and methods for obtaining same |
| US6187732B1 (en) | 1998-09-03 | 2001-02-13 | Genencor International, Inc. | Mutant EGIII cellulase, DNA encoding such EGIII compositions and methods for obtaining same |
| US6358715B1 (en) | 1998-12-04 | 2002-03-19 | Genencor International, Inc. | Production of ascorbic acid |
| US6576452B1 (en) | 2000-10-04 | 2003-06-10 | Genencor International, Inc. | 2,5-diketo-L-gluconic acid reductases and methods of use |
| CN112430560B (en) * | 2019-08-26 | 2024-01-05 | 中国科学院分子植物科学卓越创新中心 | A kind of 2-keto-L-gulonic acid production strain and its construction method |
Citations (1)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| AU2983284A (en) * | 1983-06-28 | 1985-01-03 | Genentech Inc. | Ascorbic acid intermediates and process enzymes |
Family Cites Families (2)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| JPS57186496A (en) * | 1981-05-11 | 1982-11-16 | Ajinomoto Co Inc | Preparation of l-threonine by fermentation |
| JPS60118186A (en) * | 1983-11-17 | 1985-06-25 | Shionogi & Co Ltd | 2,5-diketo-d-gluconic acid reductase |
-
1986
- 1986-08-01 AU AU62210/86A patent/AU594080B2/en not_active Ceased
- 1986-08-01 WO PCT/US1986/001571 patent/WO1987000863A1/en not_active Ceased
- 1986-08-01 DE DE8686905045T patent/DE3686041T2/en not_active Expired - Lifetime
- 1986-08-01 JP JP61504243A patent/JPH0817706B2/en not_active Expired - Lifetime
- 1986-08-01 AT AT86905045T patent/ATE78297T1/en not_active IP Right Cessation
- 1986-08-01 EP EP86905045A patent/EP0231354B1/en not_active Expired - Lifetime
-
1987
- 1987-04-02 DK DK198701694A patent/DK175120B1/en not_active IP Right Cessation
-
1994
- 1994-03-28 JP JP6057610A patent/JP2526021B2/en not_active Expired - Lifetime
-
1995
- 1995-06-28 JP JP7162718A patent/JP2577876B2/en not_active Expired - Lifetime
- 1995-06-28 JP JP7162719A patent/JP2577877B2/en not_active Expired - Lifetime
Patent Citations (1)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| AU2983284A (en) * | 1983-06-28 | 1985-01-03 | Genentech Inc. | Ascorbic acid intermediates and process enzymes |
Also Published As
| Publication number | Publication date |
|---|---|
| EP0231354A4 (en) | 1988-10-06 |
| JPH0817706B2 (en) | 1996-02-28 |
| DK175120B1 (en) | 2004-06-07 |
| JP2526021B2 (en) | 1996-08-21 |
| JPH0838185A (en) | 1996-02-13 |
| ATE78297T1 (en) | 1992-08-15 |
| JPS63500493A (en) | 1988-02-25 |
| JP2577877B2 (en) | 1997-02-05 |
| WO1987000863A1 (en) | 1987-02-12 |
| DK169487D0 (en) | 1987-04-02 |
| JPH06319564A (en) | 1994-11-22 |
| DE3686041T2 (en) | 1993-01-28 |
| EP0231354B1 (en) | 1992-07-15 |
| DK169487A (en) | 1987-04-02 |
| AU6221086A (en) | 1987-03-05 |
| DE3686041D1 (en) | 1992-08-20 |
| EP0231354A1 (en) | 1987-08-12 |
| JPH0838189A (en) | 1996-02-13 |
| JP2577876B2 (en) | 1997-02-05 |
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| MK14 | Patent ceased section 143(a) (annual fees not paid) or expired |